To test whether the basic residue clusters are important for ζ dicf localization and to identify which of the motifs is the most critical for this characteristics, we expressed in COS cells single mutated ζ molecules, changing the first RRR cluster to GGG (Proximal) or the second RRR motif to QQQ (Distal), or generated a double mutated molecule (MUT; Supporting information Fig. 1C). The results revealed that while each single mutation only partially disrupted dicf ζ localization, the double mutation almost completely abolished this localization as indicated by the dsfc/dicf ratios (Fig. 1C and Supporting Information Fig.
2). The residual minute dicf ζ found in the cells transfected with the double mutant molecule could be due to an incomplete lysis or some remaining dscf TCRs. These results suggested that ζ dicf localization buy FK506 could be conferred by its ability to directly bind actin and that a T-cell milieu is not required selleckchem to support this linkage. Since the double mutation dramatically diminished dicf ζ localization within COS cells, we further proceeded our studies focusing on the double MUT.
We next assessed the capacity of in vitro-expressed ζ wild type (WT) or (MUT) IC domains to bind actin by using a cosedimentation assay. To this end fresh actin was polymerized in the presence of different concentrations of WT or MUT-fusion proteins, and the results revealed that only the WT ζ could be precipitated with F-actin (Fig. 1D). Testing the capacity of WT and MUT ζ IC domains or peptides represent the described WT and MUT motifs, to bind F-actin showed that only the WT IC ζ protein or the peptide containing both RRR motifs could bind F-actin (Supporting Information Fig. 3). These results indicate that ζ can directly and specifically interact with F-actin, and that the positively charged motifs are crucial for this linkage. We next determined whether ζ can associate with actin within cells and assessed the involvement of its basic motifs. To this end, we used fluorescence resonance energy transfer (FRET) technology. First, to establish the
use of sensitized emission FRET, we employed cells expressing yellow fluorescent protein Non-specific serine/threonine protein kinase (YFP) conjugated to cyan fluorescent protein (CFP) as positive control and cells expressing CFP and YFP separately. FRET was detected in the positive control cells (47.4% ± 1.6) but not in the negative control cells (0%; Supporting Information Fig. 4A). Subsequently, we tagged WT and MUT ζ with YFP and actin with CFP, and expressed them in COS7 cells at the same level (Supporting Information Fig. 4B). FRET analysis was performed in order to follow the interaction between actin and WT ζ in comparison with MUT ζ. Our data indicate that WT ζ associates with actin, as demonstrated by the high FRET efficiency (27.5% ± 1.3) for this interaction (Fig. 1E). However, FRET efficiency between actin and ζ was significantly reduced (9.9% ± 1.